Method and medicine for treating huntington&#39;s disease

ABSTRACT

Provided are a method and drug for treating Huntington&#39;s disease, which includes: administering a therapeutically effective amount of a component of a plasminogen activation pathway or a related compound thereof to a subject. Also provided are a drug, pharmaceutical composition, product, and kit used for treating Huntington&#39;s disease and containing the above component or compound.

FIELD OF THE INVENTION

The present invention relates to a method for treating Huntington's disease, which includes: administering an effective amount of a component of a plasminogen activation pathway or a related compound thereof, such as plasminogen, to a subject to treat Huntington's disease.

BACKGROUND OF THE INVENTION

Huntington's disease (HD), also known as chorea major or Huntington's chorea, is a neurodegenerative disease having autosomal dominant inheritance. Its pathogenic gene is the IT-15 gene (also called the HTT gene) located at chromosome 4p16.3, which has abnormal amplification of cytosine-adenine-guanine (CAG) trinucleotide repeats in patients with Huntington's disease and has complete penetrance when the number of copies is greater than 40. Patients usually develop the disease in middle age, with main symptoms including progressive movement disorders typically characterized by dance-like symptoms, cognitive decline, and psychiatric symptoms. At present, the second-generation antipsychotic drugs, such as tetrabenazine and olanzapine, are often used to control dance-like symptoms; and antidepressants are often used to improve psychiatric symptoms such as depression. However, these drugs do not slow down the progression of the disease. Currently, some studies are actively exploring the etiological treatment through gene therapy, but there are many uncertainties in gene therapy. Therefore, how to find more effective treatment methods in another way has become the focus of research on the disease.

SUMMARY OF THE INVENTION

The present invention finds that plasminogen can significantly improve Huntington's disease and its related symptoms, for example, can improve movement disorders of a subject with Huntington's disease, improve cognitive impairment, decelerate weight loss, protect undamaged neurons, promote the repair of damaged neurons and/or improve psychiatric symptoms, which provides an effective treatment method of Huntington's disease.

The present invention relates to the following items.

1. In an aspect, the present invention relates to a method for treating Huntington's disease, which includes: administering a therapeutically effective amount of one or more compounds to a subject with Huntington's disease. The one or more compounds are selected from: a component of a plasminogen activation pathway, a compound capable of directly activating plasminogen or indirectly activating plasminogen by activating an upstream component of a plasminogen activation pathway, a compound mimicking the activity of plasminogen or plasmin, a compound capable of up-regulating the expression of plasminogen or a plasminogen activator, a plasminogen analog, a plasmin analog, a tPA or uPA analog, and an antagonist of a fibrinolysis inhibitor.

In an aspect, the present invention relates to use of one or more compounds in preparation of a drug for treating Huntington's disease. The one or more compounds are selected from: a component of a plasminogen activation pathway, a compound capable of directly activating plasminogen or indirectly activating plasminogen by activating an upstream component of a plasminogen activation pathway, a compound mimicking the activity of plasminogen or plasmin, a compound capable of up-regulating the expression of plasminogen or a plasminogen activator, a plasminogen analog, a plasmin analog, a tPA or uPA analog, and an antagonist of a fibrinolysis inhibitor.

In an aspect, the present invention relates to a drug or pharmaceutical composition for treating Huntington's disease that contains one or more compounds. The one or more compounds are selected from: a component of a plasminogen activation pathway, a compound capable of directly activating plasminogen or indirectly activating plasminogen by activating an upstream component of a plasminogen activation pathway, a compound mimicking the activity of plasminogen or plasmin, a compound capable of up-regulating the expression of plasminogen or a plasminogen activator, a plasminogen analog, a plasmin analog, a tPA or uPA analog, and an antagonist of a fibrinolysis inhibitor.

2. The method, the use, the drug or the pharmaceutical composition according to item 1, wherein the component of the plasminogen activation pathway is selected from: plasminogen, recombinant human plasmin, Lys-plasminogen, Glu-plasminogen, plasmin, a plasminogen or plasmin variant or analog containing one or more Kringle domains or protease domains of plasminogen or plasmin, mini-plasminogen, mini-plasmin, micro-plasminogen, micro-plasmin, delta-plasminogen, delta-plasmin, a plasminogen activator, tPA, and uPA.

3. The method, the use, the drug or the pharmaceutical composition according to item 1, wherein the antagonist of the fibrinolysis inhibitor is an inhibitor of PAI-1, a complement C1 inhibitor, α2 antiplasmin or an α2 macroglobulin, such as an antibody.

4. The method, the use, the drug or the pharmaceutical composition according to any one of items 1 to 3, wherein the compound has one or more effects on the subject with Huntington's disease. The one or more effects are selected from: improvement or relief of movement disorders, improvement of cognitive impairment, deceleration of weight loss, promotion of the repair of damaged neurons, improvement of neuropsychiatric symptoms, relief of anxiety, reduction of the expression of GFAP in the hippocampus, reduction of apoptosis of hippocampal cells, promotion of the recovery of the number of Nissl bodies in cerebellar, hippocampal or striatal neurons, repair of damage to the hippocampus, striatum or olfactory tubercle, promotion of the expression of BDNF in the hippocampus or striatum, and promotion of the regeneration of striatal myelin sheaths.

5. The method, the use, the drug or the pharmaceutical composition according to any one of items 1 to 4, wherein the compound is used in combination with one or more other drugs or treatment method.

6. The method, the use, the drug or the pharmaceutical composition according to item 5, wherein the other drugs or treatment methods are selected from one or more of: anti-dopaminergic drugs, dopamine receptor inhibitors, antipsychotic drugs (e.g., butyrophenone and phenothiazines), γ-aminobutyrate transaminase inhibitors, cell transplantation therapy, and gene therapy.

7. The method, the use, the drug or the pharmaceutical composition according to any one of items 1 to 6, wherein the compound is plasminogen.

8. The method, the use, the drug or the pharmaceutical composition according to any one of items 1 to 7, wherein the plasminogen is human full-length plasminogen or a conservatively substituted variant.

9. The method, the use, the drug or the pharmaceutical composition according to any one of items 1 to 7, wherein the plasminogen has at least 75%, 80%, 85%, 90%, 95%, 96%, 97%, 98% or 99% sequence identity with sequence 2, and still has the lysine binding activity or the proteolytic activity of plasminogen.

10. The method, the use, the drug or the pharmaceutical composition according to any one of items 1 to 7, wherein the plasminogen is a protein containing an amino acid sequence having at least 80%, 90%, 95%, 96%, 97%, 98% or 99% amino acid sequence identity with sequence 14 and still having the proteolytic activity of plasminogen.

11. The method, the use, the drug or the pharmaceutical composition according to any one of items 1 to 7, wherein the plasminogen is selected from: Glu-plasminogen, Lys-plasminogen, mini-plasminogen, micro-plasminogen, delta-plasminogen, and variants thereof that retain the proteolytic activity of plasminogen.

12. The method, the use, the drug or the pharmaceutical composition according to any one of items 1 to 7, wherein the plasminogen contains an amino acid sequence shown as sequence 2, 6, 8, 10 or 12, or contains a conservatively substituted variant of the amino acid sequence shown as sequence 2, 6, 8, 10 or 12.

13. The method, the use, the drug or the pharmaceutical composition according to any one of items 1 to 12, wherein the compound is administered by nasal inhalation, aerosol inhalation, nasal drops, eye drops, ear drops, an intravenous method, an intraperitoneal method, a subcutaneous method, an intracranial method, an intrathecal method, an intra-arterial method (e.g., via the carotid artery) or an intramuscular method.

In any one of the above embodiments of the present invention, the plasminogen may have at least 75%, 80%, 85%, 90%, 95%, 96%, 97%, 98% or 99% sequence identity with sequence 2, 6, 8, 10 or 12, and still have the activity, such as the lysine binding activity and the proteolytic activity, of plasminogen. In some embodiments, the plasminogen is a protein that is obtained by adding, deleting and/or substituting 1-100, 1-90, 1-80, 1-70, 1-60, 1-50, 1-45, 1-40, 1-35, 1-30, 1-25, 1-20, 1-15, 1-10, 1-5, 1-4, 1-3, 1-2 or 1 amino acid on the basis of sequence 2, 6, 8, 10 or 12, and still has the activity, such as the lysine binding activity and the proteolytic activity, of plasminogen.

In some embodiments, the plasminogen is a protein containing a plasminogen active fragment and still having the activity, such as the lysine binding activity and the proteolytic activity, of plasminogen. In some embodiments, the plasminogen is selected from Glu-plasminogen, Lys-plasminogen, mini-plasminogen, micro-plasminogen, delta-plasminogen, and variants thereof that retain the activity, such as the proteolytic activity, of plasminogen. In some embodiments, the plasminogen is natural or synthesized human plasminogen, or a variant or fragment thereof that retains the activity, such as the lysine binding activity and the proteolytic activity, of plasminogen. In some embodiments, the plasminogen is a human plasminogen ortholog from a primate or a rodent, or a variant or fragment thereof that retains the activity, such as the lysine binding activity and the proteolytic activity, of plasminogen. In some embodiments, the plasminogen has an amino acid sequence shown as sequence 2, 6, 8, 10 or 12. In some embodiments, the plasminogen is human natural plasminogen.

In some embodiments, the subject is a human. In some embodiments, the subject has the plasminogen deficiency. In some embodiments, the deficiency is congenital, secondary and/or local.

In some embodiments, the pharmaceutical composition contains a pharmaceutically acceptable carrier and plasminogen used in the above method. In some embodiments, the kit may be a preventive or therapeutic kit, which includes: (i) plasminogen used in the above method and a (ii) means for delivering the plasminogen to the subject. In some embodiments, the means is a syringe or a vial. In some embodiments, the kit also includes a label or instructions. The label or the instructions indicate that the plasminogen is administered to the subject to implement any one of the above methods.

In some embodiments, the product includes: a container with a label; and plasminogen used in the above method or a pharmaceutical composition containing plasminogen. The label indicates that the plasminogen or the composition is administered to the subject to implement any one of the above methods.

In some embodiments, the kit or the product also includes one or more other means or containers. The means or the containers contain other drugs.

In some embodiments of the above method, the plasminogen is administered systemically or locally, and preferably, the plasminogen is administered intravenously, intramuscularly or subcutaneously to the subject to treat the disease. In some embodiments of the above method, the plasminogen is administered in combination with a suitable polypeptide carrier or stabilizer. In some embodiments of the above method, the plasminogen is administered daily at a dose of 0.0001-2000 mg/kg, 0.001-800 mg/kg, 0.01-600 mg/kg, 0.1-400 mg/kg, 1-200 mg/kg, 1-100 mg/kg or 10-100 mg/kg (based on per kilogram of the body weight), or at a dose of 0.0001-2000 mg/cm², 0.001-800 mg/cm², 0.01-600 mg/cm², 0.1-400 mg/cm², 1-200 mg/cm², 1-100 mg/cm² or 10-100 mg/cm² (based on per square centimetre of the body surface area), preferably, administration is repeated at least once, and preferably, administration is performed at least daily.

The present invention explicitly covers all combinations of the technical features belonging to the embodiments of the present invention, and these combined technical solutions have been explicitly disclosed in this application, just as the above technical solutions have been separately and explicitly disclosed. In addition, the present invention also explicitly covers combinations of the embodiments and their elements, and the combined technical solutions are explicitly disclosed herein.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 shows statistical results of a total travel distance of a mouse model of Huntington's disease in an open field test after 7 days of plasminogen administration. The results show that a mouse of a blank control group travels a certain distance in the test; a total travel distance of a mouse of solvent control group is obviously longer than that of the mouse of the blank control group; a total travel distance of a mouse of a plasminogen administration group is obviously shorter than that of the mouse of the solvent control group, the statistical difference is significant (* indicates P<0.05), and the total travel distance of a mouse of the plasminogen administration group is closer to that of the mouse of the blank control group. It indicates that plasminogen can promote the recovery of spontaneous activities of the mouse model of Huntington's disease.

FIG. 2 shows statistical results of a boundary zone resting time rate of a mouse model of Huntington's disease in an open field test after 7 days of plasminogen administration. The results show that a mouse of a blank control group has a certain boundary zone resting time rate; a boundary zone resting time rate of a mouse of a solvent control group is obviously less than that of the mouse of the blank control group; a boundary zone resting time rate of a mouse of a plasminogen administration group is obviously greater than that of the mouse of the solvent control group, the statistical difference is extremely significant (*** indicates P<0.001), and the boundary zone resting time rate of the mouse of the plasminogen administration group is close to that of the mouse of the blank control group. It indicates that plasminogen can relieve anxiety behaviors of the mouse model of Huntington's disease.

FIG. 3 shows statistical results of a central zone average movement speed of a mouse model of Huntington's disease in an open field test after 7 days of plasminogen administration. The results show that a mouse of a blank control group has a certain central zone movement speed; a central zone average movement speed of a mouse of a solvent control group is obviously lower than that of the mouse of the blank control group; a central zone average movement speed of a mouse of a plasminogen administration group is obviously higher than that of the mouse of the solvent control group, the statistical difference is significant (* indicates P<0.05), and the central zone movement speed of the mouse of the plasminogen administration group is close to that of the mouse of the blank control group. It indicates that plasminogen can promote the recovery of spontaneous activities and approach-avoidance behaviors and the relief of anxiety behaviors of the mouse model of Huntington's disease.

FIG. 4 shows statistical results of a boundary zone average movement speed of a mouse model of Huntington's disease in an open field test after 7 days of plasminogen administration. The results show that a mouse of a blank control group has a certain boundary zone movement speed; a boundary zone average movement speed of a mouse of a solvent control group is obviously higher than that of the blank control group; a boundary zone average movement speed of a mouse of a plasminogen administration group is obviously lower than that of the solvent control group, the statistical difference is significant (* indicates P<0.05), and the boundary zone average movement speed of the mouse of the plasminogen administration group is close to that of the mouse of the blank control group. It indicates that plasminogen can promote the recovery of spontaneous activities and approach-avoidance behaviors and the relief of anxiety behaviors of the mouse model of Huntington's disease.

FIG. 5A to FIG. 5C are diagrams of motion trails of mouse models of Huntington's disease in an open field test after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, and C shows a plasminogen administration group. The results show that a mouse of the blank control group travels in a central zone less frequently and travels in a boundary zone more frequently, with regular motion trails; compared with the mouse of the blank control group, a mouse of the solvent group travels more frequently in the central zone and has an obviously increased total travel distance, with chaotic and irregular motion trails; a mouse of the plasminogen administration group travels less frequently in the central zone and has an obviously reduced total travel distance compared with the mouse of the solvent group, with motion trails similar to those of the mouse of the blank control group. It indicates that plasminogen can promote the recovery of spontaneous activities and approach-avoidance behaviors of the mouse model of Huntington's disease.

FIG. 6 shows calculation results of the body weight percentage of a mouse model of Huntington's disease on day 7 and day 0 after 7 days of plasminogen administration. The results show that the body weight percentage of a mouse of a blank control group is greater than 1, and the body weight tends to increase; the body weight percentage of a mouse of a solvent control group is less than that of the mouse of the blank control group; the body weight percentage of a mouse of a plasminogen administration group is obviously greater than that of the mouse of the solvent control group, and the statistical difference is close to significant (P=0.07). The results indicate that plasminogen can promote weight gain in the mouse model of Huntington's disease.

FIG. 7A to FIG. 7D show immunohistochemical staining results of GFAP in the hippocampus of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, C shows a plasminogen administration group, and D shows quantitative analysis results of the average optical density. The results show that a certain amount of GFAP is expressed in the hippocampus of a mouse of the blank control group; the expression of GFAP in the hippocampus of a mouse of the solvent control group is obviously higher than that of the mouse of the blank control group, and the statistical difference is extremely significant (*** indicates P<0.001); the expression of GFAP in the hippocampus of a mouse of the plasminogen administration group is obviously lower than that of the mouse of the solvent control group, the statistical difference is extremely significant, and there is no statistical difference between the mice of the plasminogen administration group and the blank control group in the expression of GFAP in the hippocampus. The results indicate that plasminogen can reduce the expression of GFAP in the hippocampus of the mouse model of Huntington's disease, inhibit the proliferation of astrocytes, improve the recovery of hippocampal damage.

FIG. 8A to FIG. 8D show immumohistochemical staining results of caspase-3 in the hippocampus of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, C shows a plasminogen administration group, and D shows quantitative analysis results of the average optical density. The results show that a certain amount of caspase-3 (indicated by arrows) is expressed in the hippocampus of a mouse of the blank control group; the expression of caspase-3 in the hippocampus of a mouse of the solvent control group is obviously increased; the expression of caspase-3 in the hippocampus of a mouse of the plasminogen administration group is obviously lower than that of the mouse of the solvent control group, and the statistical difference is close to significant (P=0.058). The results indicate that plasminogen can reduce the expression of caspase-3 and reduce apoptosis of hippocampal cells in the mouse model of Huntington's disease.

FIG. 9A to FIG. 9D show toluidine blue staining results of the cerebellum of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, C shows a plasminogen administration group, and D shows analysis results of the number of Nissl bodies in the cerebellum. The results show that a certain number of Nissl bodies (indicated by arrows) are present in cerebellar neurons in a mouse of the blank control group; the number of Nissl bodies in cerebellar neurons in a mouse of the solvent control group is obviously greater than that in the mouse of the blank control group; the number of Nissl bodies in cerebellar neurons in a mouse of the plasminogen administration group is obviously less than that in the mouse of the solvent control group, the statistical difference is significant (* indicates P<0.05), and there is no obvious difference between the mice of the plasminogen administration group and the blank control group. The results indicate that plasminogen can promote the recovery of the number of Nissl bodies in the cerebellar neurons in the mouse model of Huntington's disease.

FIG. 10A to FIG. 10D show cresyl violet staining results of the left hippocampus of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent group, C shows a plasminogen administration group, and D shows analysis results of the number of Nissl bodies in the hippocampus. The results show that a certain number of Nissl bodies (indicated by arrows) are present in left hippocampal neurons in a mouse of the blank control group; the number of Nissl bodies in left hippocampal neurons in a mouse of the solvent group is obviously greater than that in the mouse of the blank control group; the number of Nissl bodies in left hippocampal neurons in a mouse of the plasminogen administration group is obviously less than that in the mouse of the solvent group, and the statistical difference is significant (* indicates P<0.05). The results indicate that plasminogen can promote the recovery of the number of Nissl bodies in the hippocampal neurons.

FIG. 11A to FIG. 11D show cresyl violet staining results of the striatum of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, C shows a plasminogen administration group, and D shows analysis results of the number of Nissl bodies in the striatum. The results show that a certain number of Nissl bodies (indicated by arrows) are present in striatal neurons in a mouse of the blank control group; the number of Nissl bodies in striatal neurons in a mouse of solvent group is obviously less than that in the mouse of the blank control group; the number of Nissl bodies in striatal neurons in a mouse of the plasminogen administration group is obviously greater than that in the mouse of solvent group, and the statistical difference is significant (* indicates P<0.05). The results indicate that plasminogen can promote the recovery of the number of Nissl bodies in the striatal neurons.

FIG. 12A to FIG. 121 are H&E staining results of the hippocampus of a mouse model of Huntington's disease after 7 days of plasminogen administration. A, B, and C show a blank control group, D, E, and F show a solvent control group, and G, H, and I show a plasminogen administration group. The result show that the overall morphology of the hippocampus of a mouse of the blank control group is normal, and the structure is intact; there are disorganized neuronal arrangement, atrophy of nerve cells (indicated by thin arrows), cellular degeneration and necrosis, and sparse and edematous surrounding brain tissue (indicated by triangles) in the CA1 region, and multiple pyknotic and hyperchromatic neuronal nuclei (indicated by thick arrows) in the CA3 region of the hippocampus of a mouse of the solvent control group; the morphology of the regions of the hippocampus of a mouse of the plasminogen administration group is restored, and there are some pyknotic and hyperchromatic neuronal nuclei in the CA3 region and the DG region. The results indicate that plasminogen can repair hippocampal damage in the mouse model of Huntington's disease.

FIG. 13A to FIG. 13C show H&E staining results of the striatum of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, and C shows a plasminogen administration group. The results show that the morphological structure of the striatum of a mouse of the blank control group is normal; striatal neurons in a mouse of the solvent group are degenerated, some cell nuclei (indicated by arrows) are vacuolated, and the arrangement of brain cells is disorganized; the overall structure of the striatum of a mouse of the plasminogen administration group is significantly improved, and is similar to that of the mouse of the blank control group. The results indicate that plasminogen can repair striatal damage in the mouse model of Huntington's disease.

FIG. 14A to FIG. 14C show H&E staining results of the olfactory tubercle of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, and C shows a plasminogen administration group. The results show that the morphological structure of the olfactory tubercle of a mouse of the blank control group is normal; glial cell infiltration (indicated by arrows) in the olfactory tubercle of a mouse of the solvent group is severe; and glial cell infiltration in the olfactory tubercle of a mouse of the plasminogen administration group is obviously milder than that of the mouse of the solvent group. The results indicate that plasminogen can improve olfactory tubercle damage in the brain of the mouse model of Huntington's disease.

FIG. 15A to FIG. 15D show immumohistochemical staining results of BDNF in the hippocampus of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, C shows a plasminogen administration group, and D shows quantitative analysis results of the average optical density. The results show that a certain amount of BDNF (indicated by arrows) is expressed in the right hippocampus of a mouse of the blank control group; the expression of BDNF in the right hippocampus of a mouse of the solvent group is slightly higher than that of the mouse of the blank control group; the expression of BDNF in the right hippocampus of a mouse of the plasminogen administration group is obviously higher than that of the mouse of the solvent group, and the statistical difference is close to significant (P=0.07). The results indicate that damage can stimulate the expression of BDNF, but plasminogen can further promote the expression of BDNF, so as to promote the repair of hippocampal damage in the mouse model of Huntington's disease.

FIG. 16A to FIG. 16D show immumohistochemical staining results of BDNF in the striatum of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, C shows a plasminogen administration group, and D shows quantitative analysis results of the average optical density. The results show that a certain amount of BDNF (indicated by arrows) is expressed in the striatum of a mouse of the blank control group; the expression of BDNF in the striatum of a mouse of the solvent group is slightly higher than that of the mouse of the blank control group; the expression of BDNF in the striatum of a mouse of the plasminogen administration group is obviously higher than that of the mouse of the solvent group, and the statistical difference is close to significant (P=0.1). The results indicate that damage can stimulate the expression of BDNF, but plasminogen can further promote the expression of BDNF, so as to promote of the repair of striatal damage in the mouse model of Huntington's disease.

FIG. 17A to FIG. 17D show LFB staining results of the striatum of a mouse model of Huntington's disease after 7 days of plasminogen administration. A shows a blank control group, B shows a solvent control group, C shows a plasminogen administration group, and D shows quantitative analysis results of the average optical density. The results show that the structure of the striatal myelin sheath of a mouse of the blank control group is normal; the striatal myelin protein content in a mouse of the solvent group is decreased, and cavitation (indicates by arrows) can be observed; the striatal myelin protein content in a mouse of the plasminogen administration group is obviously greater than that in the mouse of the solvent group, and the statistical difference is close to significant (P=0.09). The results indicate that plasminogen can promote the formation of striatal myelin protein in the mouse model of Huntington's disease.

DETAILED DESCRIPTION OF THE INVENTION

Huntington's disease (HD) is a monogenic neurodegenerative disease having autosomal dominant inheritance, its pathogenesis is dominated by mHtt protein toxicity, and its main symptoms include progressive movement disorders typically characterized by dance-like symptoms, cognitive decline, and psychiatric symptoms. When a gene mutation causes an abnormal increase in the number CAG copies, an amino-terminal (N-terminal) polyglutamine chain (polyQ) of a mutant Htt (mHtt) protein can be extended to form an abnormal conformation including a lamellar structure. As a result, the mHtt protein loses normal function and gains toxicity.

The “movement disorders” in Huntington's disease are mainly divided into two types, i.e., involuntary movement disorders (dominated by chorea) and voluntary movement disorders (including uncoordinated movements and slow movements). The progressive movement disorders are characterized by sudden and rapid throbbing or twitching of the limbs, face, or trunk that is unpredictable and uncontrollable, or characterized by uncontrollable slow movements. Dance-like involuntary movements and decreased muscle tone may be detected on examination. Dance-like involuntary movements are the most prominent features of the disease, mostly starting with brief uncontrollable grimacing, nodding, and finger flexion and extension movements, similar to painless convulsions, but slower and non-stereotyped. With the progression of the disease, involuntary movements progressively worsen, typical eyebrow raising and head flexion occur, patients turn the head when staring at objects and walk unsteadily with a leaping gait and constantly changing hand posture, and the whole body moves like dance. In the later stage of the disease, patient cannot stand and walk due to involuntary movements of the whole body. With the progression of the disease, the impairment of voluntary movements becomes more pronounced, with clumsiness, slowness, and rigidity in movements, inability to maintain complex voluntary movements, dysphagia, hesitate in speech, and dysarthria. Abnormal eye movements occur. In the advanced stage of the disease, the limbs may be in a stuporous state, that is, the limbs cannot move.

The dance-like movement disorder is the typical feature of adult-onset Huntington's disease. In juvenile patients with onset before the age of 20, immobile myotonia is the main movement disorder, manifesting as myotonia, myoclonus, and opisthotonus in the later stage. In addition, differing from adult patients, about 50% of juvenile patients with Huntington's disease has the onset of systematic epilepsy.

The “cognitive impairment” in Huntington's disease can appear years before motor symptoms, and its progression is relatively slow. Progressive dementia is another feature of patients with Huntington's disease. Dementia is characterized by subcortical dementia in the early stage and characterized by mixed cortical and subcortical dementia in the later stage.

The cognitive impairment can appear in the early stage of Huntington's disease. At the beginning, patient show a decline in memory and computing abilities in daily life and work, with only mild impairments in remembering new information, but significant deficits in recall. The patients show changes in speech function, including oral disfluency, mild difficulty in finding words, and dysarthria. Impaired oral fluency is one of the earliest cognitive impairments in Huntington's disease. In the middle stage and advanced stage of the disease, patients are unable to complete a naming test that requires recall of infrequent words. Dance-like movement disorders often affect the tongue and lips to disrupt the rhythm and agility of pronunciation and interfere with the volume, speed, rhythm, and length of phrases of speech. Therefore, dysarthria and rhythm disorders are prominent features of patients with this disease.

The “neuropsychiatric symptoms” of Huntington's disease may appear very early, and may even be the first symptoms, such as depression, irritability, and apathy, while more severe symptoms include paranoia or schizophrenia-like symptoms

Fibrinolytic system is a system composed of a series of chemical substances involved in fibrinolysis. The chemical substances mainly include plasminogen, plasmin, plasminogen activators, and fibrinolysis inhibitors. The plasminogen activators include a tissue-type plasminogen activator (t-PA) and a urokinase-type plasminogen activator (u-PA). t-PA is a serine protease synthesized by vascular endothelial cells. t-PA activates plasminogen mainly on fibrin. The urokinase-type plasminogen activator (u-PA) is produced by renal tubular epithelial cells and vascular endothelial cells, and can directly activate plasminogen without the need for fibrin as a cofactor. Plasminogen (PLG) is synthesized in the liver. When blood coagulates, a large amount of PLG is adsorbed onto the fibrin network, and is activated to plasmin under the action of t-PA or u-PA to promote fibrinolysis. Plasmin (PL) is a serine protease, and has the following effects: degrading fibrin and fibrinogen; hydrolyzing a variety of blood coagulation factors such as V, VIII, X, VII, XI, and II; enabling plasminogen to be transformed into plasmin; hydrolyzing complements, etc. The fibrinolysis inhibitors include: plasminogen activator inhibitors (PAIs) and α2 antiplasmin (α2-AP). PAIs mainly include two types, i.e., PAI-1 and PAI-2, and can specifically bind to t-PA in a ratio of 1:1 to inactivate t-PA and activate PLG at the same time. α2-AP is synthesized in the liver, and binds to PL in a ratio of 1:1 to form a complex so as to inhibit the activity of PL. FXIII enables α2-AP to bind to fibrin in the form of covalent bond to attenuate the sensitivity of fibrin to the action of PL. Substances inhibiting the activity of the fibrinolytic system in vivo include: PAI-1, a complement C1 inhibitor, α2 antiplasmin, and an α2 macroglobulin.

Herein, the term “component of a plasminogen activation pathway” covers:

1. plasminogen, Lys-plasminogen, Glu-plasminogen, micro-plasminogen, delta-plasminogen, and variants and analogs thereof;

2. plasmin and variants and analogs thereof; and

3. plasminogen activators, such as tPA, uPA, and a tPA or uPA variant or analog containing one or more domains (e.g., one or more Kringle domains and proteolysis domains) of tPA or uPA.

The above “variants” of plasminogen, plasmin, tPA, and uPA include all naturally occurring human genetic variants and other mammalian forms of these proteins, and a protein that is obtained by adding, deleting and/or substituting, for example, 1-100, 1-90, 1-80, 1-70, 1-60, 1-50, 1-45, 1-40, 1-35, 1-30, 1-25, 1-20, 1-15, 1-10, 1-5, 1-4, 1-3, 1-2 or 1 amino acid and still has the activity of plasminogen, plasmin, tPA or uPA. For example, the “variants” of plasminogen, plasmin, tPA, and uPA include mutational variants of these proteins that are obtained by substituting, for example, 1-100, 1-90, 1-80, 1-70, 1-60, 1-50, 1-45, 1-40, 1-35, 1-30, 1-25, 1-20, 1-15, 1-10, 1-5, 1-4, 1-3, 1-2 or 1 amino acid with conservative amino acids.

The “plasminogen variants” of the present invention include proteins having at least 75%, 80%, 85%, 90%, 95%, 96%, 97%, 98% or 99% sequence identity with sequence 2, 6, 8, 10 or 12 and still having the activity, such as the lysine binding activity and the proteolytic activity, of plasminogen. For example, the “plasminogen variants” of the present invention may be proteins that are obtained by adding, deleting and/or substituting 1-100, 1-90, 1-80, 1-70, 1-60, 1-50, 1-45, 1-40, 1-35, 1-30, 1-25, 1-20, 1-15, 1-10, 1-5, 1-4, 1-3, 1-2 or 1 amino acid on the basis of sequence 2, 6, 8, 10 or 12 and still have the activity, such as the lysine binding activity and the proteolytic activity, of plasminogen. Specifically, the plasminogen variants of the present invention include all naturally occurring human genetic variants and other mammalian forms of these proteins, and mutational variants of these proteins that are obtained by substituting, for example, 1-100, 1-90, 1-80, 1-70, 1-60, 1-50, 1-45, 1-40, 1-35, 1-30, 1-25, 1-20, 1-15, 1-10, 1-5, 1-4, 1-3, 1-2 or 1 amino acid with conservative amino acids.

The plasminogen of the present invention may be a human plasminogen ortholog from a primate or a rodent, or a variant thereof that retains the activity, such as the lysine binding activity and the proteolytic activity, of plasminogen, such as plasminogen shown as sequence 2, 6, 8, 10 or 12, and human natural plasminogen shown as sequence 2.

The above “analogs” of plasminogen, plasmin, tPA, and uPA include compounds respectively providing functions basically similar to those of plasminogen, plasmin, tPA, or uPA.

The above “variants” and “analogs” of plasminogen, plasmin, tPA, and uPA include “variants” and “analogs” containing one or more domains (e.g., one or more Kringle domains and proteolysis domains) of plasminogen, plasmin, tPA, and uPA. For example, the “variants” and “analogs” of plasminogen include plasminogen variants and analogs containing one or more domains (e.g., one or more Kringle domains and proteolysis domains) of plasminogen, such as mini-plasminogen. The “variants” and “analogs” of plasmin include plasmin “variants” and “analogs” containing one or more domains (e.g., one or more Kringle domains and proteolysis domains) of plasmin, such as mini-plasmin and delta-plasmin (δ-plasmin).

Whether the above “variants” or “analogs” of plasminogen, plasmin, tPA or uPA have the activity of plasminogen, plasmin, tPA or uPA, or whether the above “variants” or “analogs” of plasminogen, plasmin, tPA or uPA respectively provides functions basically similar to those of plasminogen, plasmin, tPA or uPA can be detected by the methods known in the art. For example, the activity of activated plasmin is determined by enzymography, an enzyme-linked immunosorbent assay (ELISA) or fluorescence-activated cell sorting (FACS), or determined by the methods described in the following documents: Ny, A., Leonardsson, G., Hagglund, A. C, Hagglof, P., Ploplis, V. A., Carmeliet, P. and Ny, T. (1999). Ovulation inplasminogen-deficient mice. Endocrinology 140, 5030-5035; Silverstein R L, Leung L L, Harpel P C, Nachman R L (November 1984). “Complex formation of platelet thrombospondin with plasminogen. Modulation of activation by tissue activator”. J. Clin. Invest. 74 (5): 1625-33; Gravanis I, Tsirka S E (February 2008). “Tissue-type plasminogen activator as a therapeutic target in stroke”. Expert Opinion on Therapeutic Targets. 12 (2): 159-70; and Geiger M, Huber K, Wojta J, Stingl L, Espana F, Griffin J H, Binder B R (August 1989). “Complex formation between urokinase and plasma protein C inhibitor in vitro and in vivo”. Blood. 74 (2): 722-8.

In some embodiments of the present invention, the “component of the plasminogen activation pathway” of the present invention is plasminogen. In some embodiments, the plasminogen is human full-length plasminogen or a conservatively substituted variant thereof that retains the activity (e.g., the lysine binding activity and the proteolytic activity) of plasminogen. In some embodiments, the plasminogen is selected from Glu-plasminogen, Lys-plasminogen, mini-plasminogen, micro-plasminogen, delta-plasminogen, and variants thereof that retain the activity (e.g., the lysine binding activity and the proteolytic activity) of plasminogen. In some embodiments, the plasminogen is natural or synthesized human plasminogen, or a conservatively substituted variant or fragment thereof that retains the activity (e.g., the lysine binding activity and the proteolytic activity) of plasminogen. In some embodiments, the plasminogen is a human plasminogen ortholog from a primate or a rodent, or a conservatively substituted variant or fragment thereof that retains the activity of plasminogen. In some embodiments, the plasminogen contains an amino acid sequence shown as sequence 2, 6, 8, 10 or 12. In some embodiments, the plasminogen contains a conservatively substituted sequence of the amino acid sequence shown as sequence 2, 6, 8, 10 or 12. In some embodiments, the plasminogen has an amino acid sequence shown as sequence 2, 6, 8, 10 or 12. In some embodiments, the plasminogen is a conservatively substituted variant of plasminogen shown as sequence 2, 6, 8, 10 or 12. In some embodiments, the plasminogen is human natural plasminogen or a conservative mutant thereof. In some embodiments, the plasminogen is human natural plasminogen shown as sequence 2 or a conservatively substituted variant thereof.

A “compound capable of directly activating plasminogen or indirectly activating plasminogen by activating an upstream component of a plasminogen activation pathway” refers to any compound that can directly activate plasminogen or indirectly activate plasminogen by activating an upstream component of a plasminogen activation pathway, such as tPA, uPA, streptokinase, saruplase, alteplase, reteplase, tenecteplase, anistreplase, monteplase, lanoteplase, pamiteplase, and staphylokinase.

An “antagonist of a fibrinolysis inhibitor” of the present invention is a compound that antagonizes, weakens, blocks, or prevents the action of a fibrinolysis inhibitor. The fibrinolysis inhibitor is, for example, PAI-1, a complement C1 inhibitor, α2 antiplasmin or an α2 macroglobulin. The antagonist is, for example, an antibody of PAI-1, a complement C1 inhibitor, α2 antiplasmin or an α2 macroglobulin, or antisense RNA or small RNA that blocks or down-regulates the expression of PAI-1, a complement C1 inhibitor, α2 antiplasmin or an α2 macroglobulin, or a compound that occupies a binding site of PAI-1, a complement C1 inhibitor, α2 antiplasmin or an α2 macroglobulin and does not have functions of PAI-1, a complement C1 inhibitor, α2 antiplasmin or an α2 macroglobulin, or compound that blocks a binding domain and/or an activity domain of PAI-1, a complement C1 inhibitor, α2 antiplasmin or an α2 macroglobulin.

Plasmin is a key component of a plasminogen activation (PA) system. It is a broad-spectrum protease, and can hydrolyze several components, including fibrin, gelatin, fibronectin, laminin, and proteoglycans, of an extracellular matrix (ECM). In addition, plasmin can activate some matrix metalloproteinase precursors (pro-MMPs) to activate matrix metalloproteinases (MMPs). Therefore, plasmin is considered as an important upstream regulator of extracellular proteolysis. Plasmin is formed by proteolysis of plasminogen with two types of physiological PAs, i.e., a tissue-type plasminogen activator (tPA) and a urokinase-type plasminogen activator (uPA). Due to relatively high levels of plasminogen in plasma and other body fluids, it has traditionally been thought that the regulation of the PA system is mainly achieved through the synthesis and activity levels of PAs. The synthesis of components of the PA system is strictly regulated by different factors, such as a hormone, a growth factor, and a cytokine. In addition, there are specific physiological inhibitors of plasmin and PAs. A main inhibitor of plasmin is α2-antiplasmin. The activity of PAs is regulated by both of a plasminogen activator inhibitor 1 (PAI-1) for inhibiting uPA and tPA and a plasminogen activator inhibitor 2 (PAI-2) for mainly inhibiting uPA. There are uPA-specific cell surface receptors (uPARs) having the direct hydrolysis activity on the surface of some cells.

Plasminogen is a single-stranded glycoprotein, is composed of 791 amino acids, and has a molecular wight of about 92 kDa. Plasminogen is mainly synthesized in the liver, and is abundant in the extracellular fluid. The plasminogen content in plasma is about 2 μM. Therefore, plasminogen is a huge potential source of the proteolytic activity in tissues and body fluids. Plasminogen is present in two molecular forms, i.e., glutamate-plasminogen (Glu-plasminogen) and lysine-plasminogen (Lys-plasminogen). Naturally secreted and uncleaved plasminogen has an amino-terminal (N-terminal) glutamate, so it is referred to as glutamate-plasminogen. However, glutamate-plasminogen is hydrolyzed to lysine-plasminogen at Lys76-Lys77 in the presence of plasmin Compared with glutamate-plasminogen, lysine-plasminogen has higher affinity to fibrin and can be activated by PAs at a higher rate. Arg560-Va1561 peptide bonds of the two forms of plasminogen can be cleaved by uPA or tPA to form double-stranded protease plasmin linked via a disulfide bond. The amino-terminal moiety of plasminogen contains five homologous tri-circles, i.e., kringles; and the carboxyl-terminal moiety of plasminogen contains protease domains. Some kringles contain lysine binding sites for mediating specific interaction of plasminogen and fibrin, as well as its inhibitor α2-AP. It is found recently that a plasminogen fragment of 38 kDa that contains Kringle1 to Kringle4 is an effective inhibitor for angiogenesis. This fragment is named angiostatin, which can be produced by hydrolyzing plasminogen with several proteases.

A main substrate of plasmin is fibrin, and the dissolution of fibrin is a key for preventing pathological thrombosis. Plasmin also has substrate specificity to several components, including laminin, fibronectin, proteoglycans, and gelatin, of ECM, suggesting that plasmin also plays an important role in reconstruction of ECM. Indirectly, plasmin can also degrade other components, including MMP-1, MMP-2, MMP-3, and MMP-9, of ECM by transforming some protease precursors into active proteases. Therefore, it has been proposed that plasmin may be an important upstream regulator of extracellular proteolysis. In addition, plasmin has the ability to activate certain potential growth factors. In vitro, plasmin can also hydrolyze components of a complement system and release chemotactic complement fragments.

“Plasmin” is a very important enzyme present in the blood, which can hydrolyze a fibrin clot to fibrin degradation products and D-dimer.

“Plasminogen” is the zymogen form of plasmin According to sequences in Swiss Prot, a glycoprotein composed 810 amino acids, having a molecular weight of about 90 kDa, mainly synthesized in the liver, and capable of circulating in the blood is calculated based on an amino acid sequence (sequence 4) of natural human plasminogen containing a signal peptide, and a cDNA sequence for encoding the amino acid sequence is shown as sequence 3. Full-length plasminogen contains seven domains, i.e., a serine protease domain at the C terminus, a Pan Apple (PAp) domain at the N terminus, and five Kringle domains (Kringle1 to Kringle5). Referring to sequences in Swiss Prot, the signal peptide includes residues Met1-Glyl9, PAp includes residues Glu20-Va198, Kringle1 includes residues Cys103-Cys181, Kringle2 includes residues Glu184-Cys262, Kringle3 includes residues Cys275-Cys352, Kringle4 includes residues Cys377-Cys454, and Kringle5 includes residues Cys481-Cys560. According to data of NCBI, the serine protease domain includes residues Va1581-Arg804.

Glu-plasminogen is human natural full-length plasminogen and is composed of 791 amino acids (without a signal peptide of 19 amino acids), a cDNA sequence for encoding the sequence is shown as sequence 1, and an amino acid sequence of Glu-plasminogen is shown as sequence 2. In vivo, there is Lys-plasminogen formed by hydrolyzing Glu-plasminogen at amino acids at the 76th site and the 77th site, which is shown as sequence 6, and a cDNA sequence for encoding the amino acid sequence is shown as sequence 5. Delta-plasminogen (δ-plasminogen) is full-length plasminogen lacking a fragment from Kringle2 to Kringle5 and containing only Kringle1 and a serine protease domain (also referred to as a protease domain (PD)), an amino acid sequence (sequence 8) of delta-plasminogen has been reported in a document, and a cDNA sequence for encoding the amino acid sequence is shown as sequence 7. Mini-plasminogen is composed of Kringle5 and a serine protease domain, it has been reported in a document that an amino acid sequence of mini-plasminogen includes residues Va1443-Asn791 (taking a Glu residue in a sequence of Glu-plasminogen without a signal peptide as the starting amino acid), and is shown as sequence 10, and a cDNA sequence for encoding the amino acid sequence is shown as sequence 9. Micro-plasminogen contains only a serine protease domain, it has been reported in a document that an amino acid sequence of micro-plasminogen includes residues Ala543-Asn791 (taking a Glu residue in a sequence of Glu-plasminogen without a signal peptide as the starting amino acid), and it has also been reported in the patent document CN102154253A that the sequence of micro-plasminogen includes residues Lys531-Asn791 (taking a Glu residue in a sequence of Glu-plasminogen without a signal peptide as the starting amino acid). In this patent application, the amino acid sequence of micro-plasminogen is referred to the patent document CN102154253A, and is shown as sequence 12, and a cDNA sequence for encoding the amino acid sequence is shown as sequence 11.

The structure of full-length plasminogen is also described in the paper of Aisina, et al. (Aisina R B, Mukhametova L I. Structure and function of plasminogen/plasmin system W. Russian Journal of Bioorganic Chemistry, 2014, 40 (6): 590-605). In this paper, Aisina, et al. describe that plasminogen includes Kringle1, 2, 3, 4, and 5 domains and a serine protease domain (also referred to as a protease domain (PD)). Kringles are responsible for binding plasminogen to ligands having low molecular weights and high molecular weights (i.e., the lysine binding activity), so that plasminogen is transformed into a more open conformation, which can be activated more easily. The protease domain (PD) includes residues Va1562-Asn791, and tPA and uPA specifically cleave an activation bond at sites Arg561-Va1562 in plasminogen to transform plasminogen into plasmin Therefore, the protease domain (PD) is a region giving the proteolytic activity of plasminogen. Herein, the terms “plasmin”, “fibrinolysin”, and “fibrinolytic enzyme” are interchangeable and have the same meaning. The terms “plasminogen”, “profibrinolysin”, and “fibrinolytic zymogen” are interchangeable and have the same meaning.

In the present invention, the “plasminogen deficiency” means that the plasminogen content or activity in a subject is less than that in a normal person, and is low enough to affect normal physiological functions of the subject. The “plasminogen deficiency” means that the plasminogen content or activity in a subject is less than that in a normal person, the activity or expression of plasminogen is extremely low, and normal physiological functions can only be maintained by providing exogenous plasminogen.

Those in the art may understand that all technical solutions of plasminogen of the present invention are applicable to plasmin, and thus the technical solutions described in the present invention cover plasminogen and plasmin During circulation, plasminogen is in a closed inactive conformation, and is transformed into activate plasmin in an open conformation under the mediation of a plasminogen activator (PA) when binding to a thrombus or cell surface. Active plasmin can further hydrolyze a fibrin clot to fibrin degradation products and D-dimer, so as to dissolve a thrombus. The PAp domain of plasminogen contains an important determinant for maintaining plasminogen in a closed inactive conformation, and the KR domain of plasminogen can bind to a lysine residue present in a receptor and a substrate. A variety of known enzymes that can be used as plasminogen activators include: a tissue-type plasminogen activator (tPA), a urokinase-type plasminogen activator (uPA), a kallikrein, a blood coagulation factor XII (Hageman factor), etc.

A “plasminogen active fragment” refers to a fragment having the activity of binding to lysine in a target sequence of a substrate (the lysine binding activity), or the activity of exerting proteolytic function (the proteolytic activity), or the proteolytic activity and the lysine binding activity. The technical solutions related to plasminogen of the present invention cover a technical solution of replacing plasminogen with a plasminogen active fragment. In some embodiments, the plasminogen active fragment of the present invention contains the serine protease domain of plasminogen or is composed of the serine protease domain of plasminogen. In some embodiments, the plasminogen active fragment of the present invention contains sequence 14, or contains an amino acid sequence having at least 80%, 90%, 95%, 96%, 97%, 98% or 99% identity with sequence 14, or is composed of sequence 14, or is composed of the amino acid sequence having at least 80%, 90%, 95%, 96%, 97%, 98% or 99% identity with sequence 14. In some embodiments, the plasminogen active fragment of the present invention contains one or more regions selected from Kringle1, Kringle2, Kringle3, Kringle4, and Kringle5 or conservatively substituted variants thereof, or is composed of one or more regions selected from Kringle1, Kringle2, Kringle3, Kringle4, and Kringle5 or conservatively substituted variants thereof. In some embodiments, the plasminogen of the present invention includes a protein containing the above plasminogen active fragment.

At present, assays of plasminogen in the blood and its activity include: an tissue-type plasminogen activator activity assay (t-PAA), a plasma tissue-type plasminogen activator antigen assay (t-PAAg), a plasma tissue-type plasminogen activity assay (plgA), a plasma tissue plasminogen antigen assay (plgAg), a plasma tissue-type plasminogen activator inhibitor activity assay, a plasma tissue-type plasminogen activator inhibitor antigen assay, and a plasma plasmin-antiplasmin complex assay (PAP). The most commonly used test method is a chromogenic substrate method: streptokinase (SK) and a chromogenic substrate are added to plasma to be tested, PLG in the plasma to be tested is transformed into PLM under the action of SK, PLM acts on the chromogenic substrate, absorbance is measured by using a spectrophotometer, and increase in absorbance is proportional to the activity of plasminogen. In addition, immunohistochemistry, gel electrophoresis, immunoturbidimetry, radial immunodiffusion, etc. can also be adopted to test the activity of plasminogen in the blood.

An “ortholog” refers to a homolog of different species, includes a protein homolog and a DNA homolog, and is also referred to as a vertical homolog. It specifically refers to a protein or a gene in different species that has evolved from the same ancestral gene. The plasminogen of the present invention includes human natural plasminogen, and also includes plasminogen orthologs derived from different species and having the activity of plasminogen.

A “conservatively substituted variant” refers to that a given amino acid residue is changed, but the whole conformation and function of a protein or enzyme are not changed. For example, an amino acid in an amino acid sequence of a parent protein is substituted with an amino acid with similar properties (e.g., acidity, alkalinity, and hydrophobicity). The amino acid with similar properties is well known. For example, arginine, histidine, and lysine are hydrophilic alkaline amino acids and can be substituted with each other. Similarly, isoleucine is a hydrophobic amino acid and can be substituted with leucine, methionine or valine. Therefore, the similarity of amino acid sequences of two proteins having similar functions may be different. For example, 70% to 99% similarity (identity) based on the MEGALIGN algorithm. The “conservatively substituted variant” also includes a polypeptide or an enzyme that has more than 60% amino acid sequence identity determined based on BLAST or FASTA algorithm, preferably, more than 75% identity, more preferably, more than 85% identity, and the most preferably, more than 90% identity. The polypeptide or the enzyme has the same or basically similar properties or function compared to a natural or parent protein or enzyme.

“Isolated” plasminogen refers to a plasminogen protein isolated and/or recovered from a natural environment of plasminogen. In some embodiments, the plasminogen is purified (1) to the purity (by weight) of more than 90%, more than 95% or more than 98%, such as more than 99% determined by the Lowry method, (2) to an extent sufficient to obtain at least 15 residues at the N terminus or in an internal amino acid sequence by using a rotary cup sequencer, or (3) to homogeneity that is determined by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) using Coomassie blue or silver staining under reducing or non-reducing conditions. The isolated plasminogen also includes plasminogen prepared from a recombinant cell by a bioengineering technology and isolated by at least one purification step.

Herein, the terms “polypeptide”, “peptide”, and “protein” are interchangeable, refer to an aggregation form of amino acids of any length, and may include genetically encoded and non-genetically encoded amino acids, chemically or biogeochemically modified or derived amino acids, and a polypeptide having a modified peptide backbone. The terms include fusion proteins, which include, but are not limited to, a fusion protein having an heterogenous amino acid sequence, a fusion having heterogenous and homologous leader sequences (having or without an N-terminal methionine residue), etc.

“Amino acid sequence identity percentage (%)” relative to a reference polypeptide sequence is defined as, after gaps have been introduced as necessary to achieve the maximum percentage sequence identity, and no conservative substitutions are considered as a part of the sequence identity, the percentage of amino acid residues, which are identical to amino acid residues in the reference polypeptide sequence, in a candidate sequence. Comparison for determining percentage amino acid sequence identity can be achieved in a variety of ways within the technical scope of the art. For example, software available to the public, such as BLAST, BLAST-2, ALIGN, and Megalign (DNASTAR), is adopted. Those skilled in the art can determine appropriate parameters used for comparing sequences, such as any algorithm needed to achieve the maximum comparison over the full lengths of sequences to be compared. However, for the purpose of the present invention, an amino acid sequence identity percentage value is generated by using the sequence comparison computer program ALIGN-2.

In a case that ALIGN-2 is adopted to compare amino acid sequences, % amino acid sequence identity of a given amino acid sequence A relative to a given amino acid sequence B (or may be expressed as that the given amino acid sequence A has or contains certain % amino acid sequence identity relative to, with, or to the given amino acid sequence B) is calculated as follows:

X/Y×100%

where, X is the number of amino acid residues, identically matched with amino acid residues in B, in A that is determined by the sequence comparison program ALIGN-2, and Y is the total number of amino acid residues in B. It is to be understood that in a case that the length of the amino acid sequence A differs from that of the amino acid sequence B, % amino acid sequence identity of A relative to B is not equal to % amino acid sequence identity of B relative to A. Unless otherwise specifically described, all % amino acid sequence identity values used herein are obtained by using the ALIGN-2 computer program as described in the preceding paragraph.

As used herein, the term “treatment” refers to obtaining a desired pharmacological and/or physiological effect. The effect may be complete or partial prevention of occurrence and onset of a disease or its symptoms, partial or complete alleviation of a disease and/or its symptoms, and/or partial or complete cure of a disease and/or its symptoms, which includes: (a) prevention of occurrence or onset of a disease in a subject who may have a predisposition to the disease but has not been diagnosed with the disease; (b) inhibition of a disease, i.e., retardation of the formation of the disease; and (c) alleviation of a disease and/or its symptoms, i.e. subsidence or disappearance of the disease and/or its symptoms.

Herein, the terms “individual”, “subject”, and “patient” are interchangeable, and refer to a mammal, which includes, but is not limited to, murine (rats and mice), non-human primates, humans, dogs, cats, ungulates (e.g., horses, cattle, sheep, pigs, and goats), etc.

A “therapeutically effective amount” or “effective dose” refers to an amount of a component of a plasminogen activation pathway or its related compound (e.g., plasminogen) that is sufficient to prevent and/or treat a disease when administered to a mammal or other subjects to treat the disease. The “therapeutically effective amount” is changed with the component of the plasminogen activation pathway or its related compound (e.g., plasminogen) used, a disease of a subject to be treated and/or the severity of symptoms, age, and weight, etc.

Preparation of the plasminogen of the present invention

Plasminogen can be isolated from nature and purified for further therapeutic use, or can be synthesized by a standard chemical peptide synthesis technology. In a case that a polypeptide is synthesized chemically, plasminogen can be synthesized from a liquid phase or a solid phase. Solid-phase polypeptide synthesis (SPPS) (in which a C-terminal amino acid of a sequence is attached to an insoluble support, followed by sequential addition of the remaining amino acids in the sequence) is a method suitable for chemical synthesis of plasminogen. Various SPPS methods, such as Fmoc and Boc, can be used to synthesize plasminogen. The solid-phase synthesis technique is described in Barany, et al. Solid-Phase Peptide Synthesis; The Peptides: Analysis, Synthesis, Biology. Vol. 2: Special Methods in Peptide Synthesis, Part A, 3-284; Merrifield. Solid Phase Peptide Synthesis. I. The Synthesis of a Tetrapeptide. J. Am. Chem. Soc., 85: 2149-2156 (1963); Stewart, et al. Solid Phase Peptide Synthesis, 2nd ed. Pierce Chem. Co., Rockford, Ill. (1984); Ganesan A. 2006 Mini Rev. Med Chem. 6: 3-10; and Camarero J A, et al. 2005 Protein Pept Lett. 12: 723-8. In short, small insoluble porous beads are treated with a functional unit on which a peptide chain is built. After recirculation of coupling/deprotection, the attached solid-phase free N-terminal amine is coupled to a single N-protected amino acid unit. This unit is then deprotected to reveal a new N-terminal amine that can be attached to another amino acid. The peptide remains immobilized on the solid phase and then is cleaved.

The plasminogen of the present invention can be produced by a standard recombination method. For example, a nucleic acid for encoding plasminogen is inserted into an expression vector so as to be operably connected to a regulatory sequence in the expression vector. The expression regulatory sequence includes, but is not limited to, a promoter (e.g., a naturally related or heterogenous promoter), a signal sequence, an enhancer element, and a transcription termination sequence. The expression regulatory sequence may be a eukaryotic promoter system in the vector, and the vector can transform or transfect eukaryotic host cells (e.g., COS or CHO cells). Once the vector is incorporated into a suitable host, the vector maintains the host under conditions suitable for high expression of a nucleotide sequence and collection and purification of plasminogen.

The suitable expression vector usually replicates in the host organism as an episome or an integrated part of the host chromosomal DNA. Normally, the expression vector contains a selectable marker (e.g., ampicillin resistance, hygromycin resistance, tetracycline resistance, kanamycin resistance, and neomycin resistance) to facilitate detection of cells transformed with an exogenous desired DNA sequence.

Exemplary prokaryotic host cells that can be used to clone a polynucleotide for encoding a subject antibody include Escherichia coli. Other suitable microbial hosts include: Bacillus such as Bacillus subtilis, and other Enterobacteriaceae such as Salmonella, Serratia, and various Pseudomonas species. Expression vectors can also be generated in these prokaryotic hosts, and usually contain expression control sequences (origin of replication) compatible with the host cells. In addition, there are many known promoters, such as a lactose promoter system, a tryptophan (trp) promoter system, a beta-lactamase promoter system, and a promoter system from bacteriophage λ. The promoter usually controls expression optionally in a sequence of an operator gene, and has a ribosome binding site sequence for initiating and completing transcription and translation.

Other microorganisms, such as yeast, can also be used for expression. Exemplary suitable yeast host cells include yeast (e.g., Saccharomyces cerevisiae (S. cerevisiae)) and Pichia, and the suitable vector has an expression control sequence (e.g., a promoter), origin of replication, a terminator sequence, etc. according to the requirements. Typical promoters contain 3-phosphoglycerate kinase and other glycogenolysis enzymes. Inducible yeast promoters specially include promotes from alcohol dehydrogenase, hetero-cytochrome C, and enzymes responsible for using maltose and galactose.

In addition to microorganisms, mammalian cells (e.g., mammalian cells cultured in a cell culture medium in vitro) can also be used for expressing and generating the anti-Tau antibody (e.g., a polynucleotide for encoding a subject anti-Tau antibody) of the present invention. Referring to Winnacker, From Genes to Clones, VCH Publishers, N.Y., N.Y. (1987). Suitable mammal host cells include a CHO cell line, various Cos cell line, HeLa cells, a myeloma cell line, and transformed B cells or hybridoma. An expression vector used for these cells may include an expression control sequence such as origin of replication, a promoter, and an enhancer (Queen, et al. Immunol. Rev. 89: 49 (1986)), and a necessary information processing site such as a ribosome binding site, an RNA splicing site, a polyadenylation site, and a transcription terminator sequence. Exemplary suitable expression control sequences include derived promoters such as a white immunoglobulin gene, SV40, an adenovirus, a bovine papillomavirus, and a cytomegalovirus. Referring to Co, et al. J. Immunol. 148: 1149 (1992).

Once the plasminogen of the present invention is synthesized (by the chemical or recombination method), the plasminogen of the present invention is purified in accordance with the standard procedure in the art, which includes ammonium sulfate precipitation, affinity column, column chromatography, high performance liquid chromatography (HPLC), gel electrophoresis, etc. The plasminogen is substantially pure, for example, at least about 80% to 85% pure, at least 85% to 90% pure, at least about 90% to 95% pure, 98% to 99% pure or purer. For example, the plasminogen does not contain contaminants such as cellular debris and macromolecules other than the target product.

Drug Preparation

A therapeutic preparation is a lyophilized preparation or an aqueous solution formed by mixing plasminogen with required purity with an optional pharmaceutical carrier, excipient or stabilizer (Remington's Pharmaceutical Sciences, 16th edition, Osol, A. ed. (1980)). The acceptable carrier, excipient or stabilizer at a used dose and concentration is nontoxic to subjects, and includes a buffer such as phosphates, citrates, and other organic acids; an antioxidant such as ascorbic acid and methionine; a preservative (e.g., octadecyl dimethyl benzyl ammonium chloride, hexanediamine chloride, benzalkonium chloride, benzethonium chloride, phenol, butanol, benzyl alcohol, alkyl parabens such as methyl and ethyl parabens, catechol, resorcinol, cyclohexanol, 3-pentanol, and m-cresol); a polypeptide with a low molecular weight (less than about 10 residues); a protein such as serum albumin, gelatin, and immunoglobulin; a hydrophilic polymer such as polyvinylpyrrolidone; an amino acid such as glycine, glutamine, asparagine, histidine, arginine, and lysine; monosaccharide, disaccharide, and other carbohydrates such as glucose, mannose, and dextrin; a chelant such as EDTA; saccharides such as sucrose, mannitol, fucose, and sorbitol; salt-forming counterions such as sodium; a metal complex (e.g., a zinc-protein complex); and/or a non-ionic surfactant such as TWEEN™, PLURONICS™, and polyethylene glycol (PEG). A preferred lyophilized anti-VEGF antibody preparation is described in WO 97/04801, which is incorporated herein by reference.

The preparation of the present invention may also contain more than one active compound needed for treating a specific symptom, and preferably, the active compounds are complementary and do not have side effects on each other. For example, antihypertensive drugs, antiarrhythmic drugs, and drugs for treating diabetes.

The plasminogen of the present invention can be encapsulated in a microcapsule prepared by techniques such as coacervation or interfacial polymerization, for example, can be placed in a colloidal drug delivery system (e.g., a liposome, an albumin microsphere, a microemulsion, nanoparticles, and a nanocapsule) or placed in hydroxymethylcellulose in a macroemulsion or a gel-microcapsule and a poly-(methyl methacrylate) microcapsule. These techniques are disclosed in Remington's Pharmaceutical Sciences 16th edition, Osol, A. Ed. (1980).

The plasminogen of the present invention that is used for in vivo administration needs to be sterile. It can be easily achieved by filtration with a sterile filter before or after lyophilization and re-preparation.

The plasminogen of the present invention can be used in preparation of a sustained-release preparation. Exemplary suitable sustained-release preparations include semipermeable matrices of solid hydrophobic polymers having a shape and containing glycoproteins, such as membranes or microcapsules. Exemplary sustained-release matrices include polyesters, hydrogels (e.g., poly(2-hydroxyethyl-methacrylate) (Langer, et al. J. Biomed. Mater. Res., 15: 167-277 (1981); Langer, Chem. Tech., 12: 98-105 (1982)) or polyvinyl alcohol, polylactide (U.S. Pat. No. 3,773,919, EP 58,481), L-glutamic acid, and a γ ethyl-L-glutamic acid copolymer (Sidman, et al. Biopolymers 22: 547 (1983)), non-degradable ethylene-vinyl acetate (Langer, et al. same as above) or degradable lactic acid-glycolic acid copolymer such as Lupron Depot™ (an injectable microsphere composed of a lactic acid-glycolic acid copolymer and leuprolide acetate), and poly-D-(−)-3-hydroxybutyric acid. The copolymers, such as ethylene-vinyl acetate and lactic acid-glycolic acid, can sustainably release molecules for more than 100 days, and some hydrogels release proteins for a short time period. Rational strategies for stabilizing proteins can be designed based on the relevant mechanisms. For example, in a case that the mechanism of coacervation is formation of intermolecular S—S bonds through the exchange of thiodisulfide bonds, proteins can be stabilized by modifying sulfhydryl residues, lyophilizing from an acid solution, controlling humidity, using an appropriate additive, and developing a specific polymer matrix composition.

Administration and Dosage

The pharmaceutical composition of the present invention can be administered by different methods, such as nasal inhalation, aerosol inhalation, nasal drops or eye drops, an intravenous method, an intraperitoneal method, a subcutaneous method, an intracranial method, an intrathecal method, an intraarterial method (e.g., via the carotid artery), an intramuscular method, and a rectal administration.

Preparations for parenteral administration include sterile aqueous or non-aqueous solutions, suspensions, and emulsions. Non-aqueous solvents include propylene glycol, polyethylene glycol, vegetable oils such as olive oil, and injectable organic esters such as ethyl oleate. Aqueous vectors include water, alcoholic/aqueous solutions, emulsions, and suspensions such as saline and a buffer medium. Parenteral intermedia include a sodium chloride solution, Ringer's dextrose, dextrose, sodium chloride, and fixed oils. Intravenous intermedia include fluids and nutritional supplements, electrolyte supplements, etc. A preservative and other additives, such as an antimicrobial, an antioxidant, a chelator, and inert gas, may be present.

Medical staffs will determine a dosage regimen based on various clinical factors. As well known in the medical field, a dosage regimen for any patient is determined according to a variety of factors, including the body size of a patient, the body surface area, age, a specific compound to be administered, sex, the frequency and path of administration, general health conditions, and other drugs to be administered together. A daily dosage range of the pharmaceutical composition containing plasminogen of the present invention may be, for example, about 0.0001-2000 mg/kg, or about 0.001-500 mg/kg (e.g., 0.02 mg/kg, 0.25 mg/kg, 0.5 mg/kg, 0.75 mg/kg, 10 mg/kg, and 50 mg/kg) of body weight of a patient. For example, a dose may be 1 mg/kg of body weight or 50 mg/kg of body weight, or within a range of 1-50 mg/kg of body weight, or at least 1 mg/kg of body weight. Doses greater or less than these exemplary ranges are also covered, especially in view of the above factors. Intermediate doses within the above ranges also fall within the scope of the present invention. Subjects may be administered with the pharmaceutical composition at such doses daily, every other day, weekly, or according to any other regimen determined by empirical analysis. Exemplary dosage regimens include that the pharmaceutical composition is administered at 0.01-100 mg/kg for consecutive days. It is necessary to assess a therapeutic effect and the safety during administration with the drug of the present invention.

Product or Kit

An embodiment of the present invention relates to a product or kit, which includes the plasminogen or plasmin of the present invention that is used to treat cardiovascular diseases caused by diabetes and related symptoms thereof. Preferably, the product includes a container with a label or package insert. Suitable containers include bottles, vials, syringes, etc. The container can be made from a variety of materials such as glass and plastic. The container contains a composition that can be used to treat the disease or symptoms of the present invention, and has a sterile inlet (e.g. the container may be an intravenous solution pack or vial with a plug that can be penetrated by a hypodermic needle). At least one active ingredient in the composition is plasminogen/plasmin. The label attached to the container is used to describe that the composition is used to treat the cardiovascular diseases caused by diabetes and related symptoms thereof of the present invention. The product may also include a second container containing a medicinal buffer such as phosphate-buffered saline, a Ringer's solution, and a dextrose solution. The product may also include other substances required from a commercial and user standpoint, which include other buffers, a diluent, a filter, a needle, and a syringe. In addition, the product includes a package insert with instructions for use, which are used to, for example, indicate a user of the composition to administer the plasminogen composition and other drugs for treating concomitant diseases to a patient.

EXAMPLES

Human plasminogen used in all the following examples was from plasma of a human donator, that is, was isolated from plasma of a human donator and purified by a method optimized with reference to the methods described in the following documents: Kenneth C Robbins, Louis Summaria, David Elwyn, et al. Further Studies on the Purification and Characterization of Human Plasminogen and Plasmin Journal of Biological Chemistry, 1965, 240 (1): 541-550; Summaria L, Spitz F, Arzadon L, et al. Isolation and characterization of the affinity chromatography forms of human Glu- and Lys-plasminogens and plasmins J Biol Chem. 1976 Jun. 25; 251 (12): 3693-9; HAGAN JJ, ABLONDI FB, DE RENZO EC. Purification and biochemical properties of human plasminogen. J Biol Chem. 1960 April; 235: 1005-10. The purity of plasminogen monomers was greater than 98%.

Example 1 Plasminogen Improves Spontaneous Activities and Approach-Avoidance Behaviors of a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simply open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mice of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]). Preparation of the 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice of the model group in the open field test. A solvent (a 10 mM sodium citrate solution, pH=7.4) was injected into each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day [v1], and administration was performed for 7 consecutive days. An open field test was performed on day 7 of administration.

3-NP is a natural mycotoxin, which can irreversibly inhibit mitochondrial succinate dehydrogenase, cross the blood-brain barrier to cause neurotoxicity, cause neuronal death, and mimic human HD symptoms^([1].)

Open Field Test

In the test, the mouse was placed in the central of the bottom of the open field (40×40×40 cm) while video recording and timing were performed at the same time. The mouse was continuously observed for 5 min, and 3 tests were performed on each mouse. The Smart system is a complete and user-friendly video tracking system for assessing behaviors of an experimental animal. It records trajectories, activities, specific behaviors (e.g., rotation, stretching, and feeding), and events, and calculates various analysis parameter. The test used the Smart3.0 system to record and analyze motions of the mice, and parameters included a total travel distance, a boundary zone resting time rate, a central zone average movement speed, and a boundary zone average movement speed. In each test, the box was wiped with 70% ethanol to prevent the preference caused by odor^([1].)

The open field test is designed based on the phobotaxis of mice, which means that mice are afraid of open, unknown, and potentially dangerous places, and thus have a natural tendency to move “against the wall”. The phobotaxis is assessed based on activities of the mouse in surrounding zones (four corners and four sides) of the open field. In view of duration in the surrounding zones that reflects the phobotaxis, if the duration is shorter, the mouse is more “adventurous”. If the duration in the central zone is longer, the phobotaxis and the anxiety (depression) level are lower.

Total Travel Distance

A total travel distance refers to the length of motion trails within the specified test time. The results show that in the test, the mouse of the blank control group travels a certain distance; a total travel distance of the mouse of the solvent control group is obviously longer than that of the mouse of the blank control group; a total travel distance of the mouse of the plasminogen administration group is obviously shorter than that of the mouse of the solvent control group, the statistical difference is significant (* indicates P<0.05), and the total travel distance of the mouse of the plasminogen administration group is close to that of the mouse of the blank control group (see FIG. 1 ). It indicates that plasminogen can promote the recovery of spontaneous activities of the mouse model of Huntington's disease.

Boundary Zone Resting Time Rate

Boundary zones are surrounding zones (for corners and four sides) of the open field. A boundary zone resting time rate refers to a ratio of boundary zone resting time to total resting time (including boundary zone resting time and central zone resting time). The results show that the mouse of the blank control group has a certain boundary zone resting time rate; a boundary zone resting time rate of the mouse of the solvent control group is obviously less than that of the mouse of the blank control group; a boundary zone resting time rate of the mouse of the plasminogen administration group is obviously greater than that of the mouse of the solvent control group, the statistical difference is extremely significant (*** indicates P<0.001), and the boundary zone resting time rate of the mouse of the plasminogen administration group is close to that of the mouse of the blank control group (see FIG. 2 ). It indicates that plasminogen can relieve anxiety behaviors of the mouse model of Huntington's disease.

Central Zone Average Movement Speed

A central zone refers to a zone (20×20 cm) in the centre of the open field. A central zone average movement speed refers to a ratio of a central zone travel distance to total central zone duration (including travelling and resting time). The results show that the mouse of the blank control group has a certain central zone movement speed; a central zone average movement speed of the mouse of the solvent control group is obviously lower than that of the mouse of the blank control group; a central zone average movement speed of the mouse of the plasminogen administration group is obviously higher than that of the mouse of the solvent control group, the statistical difference is significant (* indicates P<0.05), and the central zone average movement speed of the mouse of the plasminogen administration group is close to that of the mouse of the blank control group (see FIG. 3 ). It indicates that plasminogen can promote spontaneous activities and relieve anxiety behaviors of the mouse model of Huntington's disease.

Boundary Zone Average Movement Speed

A boundary zone average movement speed refers to a ratio of a total boundary zone travel distance to total boundary zone duration. The results show that the mouse of the blank control group has a certain boundary zone movement speed; a boundary zone average movement speed of the mouse of the solvent control group is obviously higher than that of the mouse of the blank control group; a boundary zone average movement speed of the mouse of the plasminogen administration group is obviously lower than that of the mouse of the solvent control group, the statistical difference is significant (* indicates P<0.05), and the boundary zone average movement speed of the mouse of the plasminogen administration group is close to that of the mouse of the blank control group (see FIG. 4 ). It indicates that plasminogen can promote spontaneous activities and relieve anxiety behaviors of the mouse model of Huntington's disease.

Motion Trail

The results show that the mouse of the blank control group (see FIG. 5A) travels in the central zone less frequently and travels in the boundary zone more frequently, with regular motion trails; compared with the mouse of the blank control group, the mouse of the solvent group (see FIG. 5B) travels more frequently in the central zone and has an obviously increased total travel distance, with chaotic and irregular motion trails; the mouse of the plasminogen administration group (see FIG. 5C) travels less frequently in the central zone and has an obviously reduced total travel distance compared with the mouse of the solvent group, with motion trails similar to those of the mouse of the blank control group. It indicates that plasminogen can promote the recovery of spontaneous activities and approach-avoidance behaviors of the mouse model of Huntington's disease.

Example 2 Plasminogen Decelerates Weight Loss in a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]). Preparation of the 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were weighed on day 7 of administration, and the body weight percentage of each mouse was calculated on day 7 and day 0.

Weight loss is a common non-neural phenotype of Huntington's disease that is usually progressive and can lead to malnutrition or cachexia^([5]).

The results show that the body weight percentage of the mouse of the blank control group is greater than 1, and the body weight tends to increase; the body weight percentage of the mouse of the solvent control group is less than that of the mouse of the blank control group; the body weight percentage of the mouse of the plasminogen administration group is obviously greater than that of the mouse of the solvent control group, and the statistical difference is close to significant (P=0.07). (FIG. 6 ) The results indicate that plasminogen can promote weight gain in the mouse model of Huntington's disease.

Example 3 Plasminogen Reduces the Expression of GFAP in the Hippocampus of a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]. Preparation of the) 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (10 mM citric acid-sodium citrate, pH=7.4) was injected into each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, the hippocampus was taken out and fixed in a 10% formaldehyde solution for 24-48 h. The fixed hippocampus tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 3 μm, and the slice was subjected to deparaffinage and rehydration, and washed once with water. The tissue slice was marked by using a PAP pen, incubated in 3% hydrogen peroxide for 15 min, and washed twice with 0.01 M PBS for 5 min each time. The slice was blocked with a 5% normal goat serum (Vector laboratories, Inc., USA) for 30 min; and then, the goat serum was removed, a rabbit anti-GFAP antibody (Abcam, ab7260) was added dropwise, and the slice was incubated at 4° C. overnight and washed twice with 0.01 M PBS for 5 min each time. A goat anti-rabbit IgG (HRP) antibody (Abcam) secondary antibody was added, and the slice was incubated at the room temperature for 1 h and washed twice with 0.01 M PBS for 5 min each time. The slice was developed by using a DAB kit (Vector laboratories, Inc., USA), washed three times with water, restained with hematoxylin for 30 s, and rinsed with running water for 5 min. The stained slice was dehydrated with graded ethanol, cleared with xylene, sealed by a neutral gum, and observed under a 400×optical microscope.

Glial fibrillary acidic protein (GFAP) is a typical intermediate filament protein in an astrocyte, which is involved in the formation of a cytoskeleton and maintenance of the strength of the cytoskeleton. Astrocytes are one of main glial cells in the central nervous system, and studies have revealed that Huntington's disease is accompanied with the proliferation of astrocytes and improvement of the activity of astrocytes, which are characterized by up-regulation of the expression of GFAP and cellular hypertrophy^([6-7]).

The results show that a certain amount of GFAP is expressed in the hippocampus of the mouse of the blank control group (see FIG. 7A); the expression of GFAP in the hippocampus of the mouse of the solvent control group (see FIG. 7B) is obviously higher than that of the mouse of the blank control group, and the statistical difference is extremely significant (*** indicates P<0.001) (see FIG. 7D); the expression of GFAP in the hippocampus of the mouse of the plasminogen administration group (see FIG. 7C) is obviously lower than that of the mouse of the solvent control group, the statistical difference is significant, and there is no statistical difference between the mice of the plasminogen administration group and the blank control group in the expression of GFAP in the hippocampus. The results indicate that plasminogen can reduce the expression of GFAP in the hippocampus of the mouse model of Huntington's disease, can inhibit the proliferation of astrocytes, and has neuroprotective effects.

Example 4 Plasminogen Reduces Apoptosis of Hippocampal Cells in a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]). Preparation of the 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, and the hippocampus was taken out and fixed in a 10% neutral formaldehyde solution for 24-48 h. The fixed hippocampus tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 3 μm, and the slice was subjected to deparaffinage and rehydration, and washed once with water. The tissue slice was marked by using a PAP pen, incubated in 3% hydrogen peroxide for 15 min, and washed twice with 0.01 M PBS for 5 min each time. The slice was blocked with a 5% normal goat serum (Vector laboratories, Inc., USA) for 30 min; and then, the goat serum was removed, a rabbit anti-caspase-3 antibody (Boster Biological Technology, BA2142) was added dropwise, and the slice was incubated at 4° C. overnight and washed twice with 0.01 M PBS for 5 min each time. A goat anti-rabbit IgG (HRP) antibody (Abcam) secondary antibody was added, and the slice was incubated at the room temperature for 1 h and washed twice with 0.01 M PBS for 5 min each time. The slice was developed by using a DAB kit (Vector laboratories, Inc., USA), washed three times with water, restained with hematoxylin for 30 s, and rinsed with running water for 5 min. The stained slice was dehydrated with graded ethanol, cleared with xylene, sealed by a neutral gum, and observed under a 400×optical microscope.

The caspase family plays a very important role in mediating apoptosis, with caspase-3 being a key executive molecule, which functions in many apoptosis signaling pathways. In a model of 3-NP Huntington's disease, neuronal apoptosis is increased and the expression of caspase-3 is up-regulated.

The results show that a certain amount of caspase-3 (indicated by arrows) is expressed in the hippocampus of the mouse of the blank control group (see FIG. 8A); the expression of caspase-3 in the hippocampus of the mouse of the solvent control group (see FIG. 8B) is obviously increased; the expression of caspase-3 in the hippocampus of the mouse of the plasminogen administration group (see FIG. 8C) is obviously less than that of the mouse of the solvent control group, and the statistical difference is close to significant (P=0.058) (see FIG. 8D). The results indicate that plasminogen can reduce the expression of caspase-3 and reduce apoptosis of hippocampal cells in the mouse model of Huntington's disease.

Example 5 Plasminogen Promotes the Recovery of the Number of Nissl Bodies in Cerebellar Neurons in a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]). Preparation of the 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, the cerebellum was taken out and fixed in a 10% neutral formaldehyde solution for 24-48 h. The fixed cerebellum was dehydrated with degraded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 3 μm, and the slice was subjected to deparaffinage and rehydration, and stained with a 0.5% toluidine blue dye. The stained slice was dehydrated with graded ethanol, cleared with xylene, and sealed by a neutral gum. The slice was observed and photographed under an optical microscope.

Nissl bodies are one of characteristic structures of neurons and are synthesis site of structural proteins and functional proteins of neurons, and their quantity and distribution are closely related to the functional state of neurons. Main chemical components of a Nissl body are ribonucleic acid and protein, Nissl bodies also called extranuclear chromatin and have affinity to basic dyes such as toluidine blue, thionine, and cresyl violet. Toluidine blue staining is the most commonly used conventional method for developing Nissl bodies^([8]). When a nervous system disease occurs, the state of Nissl bodies will be abnormal.

The results show that a certain number of Nissl bodies (indicated by arrows) are present in cerebellar neurons in the mouse of the blank control group (see FIG. 9A); the number of Nissl bodies in cerebellar neurons in the mouse of the solvent control group (see FIG. 9B) is obviously greater than that in the mouse of the blank control group; the number of Nissl bodies in cerebellar neurons in the mouse of the plasminogen administration group (see FIG. 9C) is obviously less than that in the mouse of the solvent control group, the statistical difference is significant (* indicates P<0.05) (see FIG. 9D), and there is no obvious difference between the mice of the plasminogen administration group and the blank control group in the number of Nissl bodies in cerebellar neurons. The results indicate that plasminogen cam promote the recovery of the number of Nissl bodies in cerebellar neurons of the mouse model of Huntington's disease.

Example 6 Plasminogen Promotes the Recovery of the Number of Nissl Bodies in Hippocampal Neurons in a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]. Preparation of the) 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, and the hippocampus was taken out and fixed in a 10% neutral formaldehyde solution for 24-48 h. The fixed hippocampus tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 3 μm, and the slice was subjected to deparaffinage and rehydration, and stained with a 0.4% cresyl violet dye (pH=3, manufacturer: Sinopharm Chemical Reagent Co., Ltd., batch number: 20181019). The stained slice was dehydrated with graded ethanol, cleared with xylene, and sealed by a neutral gum. The slice was observed and photographed under a 400×optical microscope.

Cresyl violet staining uses cresyl violet as a core dye. Cresyl violet has a photosensitive effect and can well show changes of Nissl bodies.

The results show that a certain number of Nissl bodies (indicated by arrows) are present in the left hippocampus of the mouse of the blank control group (see FIG. 10A); the number of Nissl bodies in the left hippocampus of the mouse of the solvent group (see FIG. 10B) is obviously greater than that of the mouse of the blank control group; the number of Nissl bodies in the left hippocampus of the mouse of the plasminogen administration group (see FIG. 10C) is obviously less than that of the mouse of the solvent group, and the statistical difference is significant (* indicates P<0.05) (see FIG. 10D). The results indicate that plasminogen can promote the recovery of the number of Nissl bodies in hippocampal neurons.

Example 7 Plasminogen Promotes the Recovery of the Number of Nissl Bodies in Striatal Neurons in a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]. Preparation of the) 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, the striatum was taken out and fixed in a 10% neutral formaldehyde solution for 24-48 h. The fixed striatum tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 3 μm, and the slice was subjected to deparaffinage and rehydration, and stained with a 0.4% cresyl violet dye (pH=3). The stained slice was dehydrated with graded ethanol, cleared with xylene, and sealed by a neutral gum. The slice was observed and photographed under a 400×optical microscope.

The results show that a certain number of Nissl bodies are present in striatal neurons in the mouse of the blank control group (see FIG. 11A); the number of Nissl bodies in striatal neurons in the mouse of the solvent group (see FIG. 11B) is obviously less than that of the mouse of the blank control group; the number of Nissl bodies in striatal neurons in the mouse of the plasminogen administration group (see FIG. 11C) is obviously greater than that of the mouse of the solvent group, and the statistical difference is significant (* indicates P<0.05) (see FIG. 11D). The results indicate that plasminogen can promote the recovery of the number of Nissl bodies in the striatal neurons.

Example 8 Plasminogen Reduces Hippocampal Damage in a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]). Preparation of the 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, the hippocampus was taken out and fixed in a 10% formaldehyde solution for 24-48 h. The fixed hippocampus tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 4 μm, and the slice was subjected to deparaffinage and rehydration, stained with hematoxylin and eosin (HE staining), differentiated with 1% hydrochloride ethanol, returned to blue with ammonia water, dehydrated with graded ethanol, sealed, and observed under a 200×optical microscope.

The results show that the overall morphology of the hippocampus of the mouse of the blank control group (see FIG. 12A to FIG. 12C), and the structure is intact; there are disorganized neuronal arrangement, atrophy of nerve cells (indicated by thin arrows), cellular degeneration and necrosis, and sparse and edematous surrounding brain tissue (indicated by triangles) in the CA1 region, and multiple pyknotic and hyperchromatic neuronal nuclei (indicated by thick arrows) in the CA3 region of the hippocampus of the mouse of the solvent control group (see 12D to FIG. 12F); the morphology of the regions of the hippocampus of the mouse of the plasminogen administration (see FIG. 12G to FIG. 12I) group is restored, and there are some pyknotic and hyperchromatic neuronal nuclei in the CA3 region and the DG region. The results indicate that plasminogen can repair hippocampal damage in the mouse model of Huntington's disease.

Example 9 Plasminogen Reduces Striatal Damage in a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]). Preparation of the 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, the striatum was taken out and fixed in a 10% neutral formaldehyde solution for 24-48 h. The fixed striatum tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 3 μm, and the slice was subjected to deparaffinage and rehydration, stained with hematoxylin and eosin (HE staining), differentiated with 1% hydrochloride ethanol, returned to blue with ammonia water, dehydrated with graded ethanol, sealed, and observed under a 200×optical microscope.

The results show that the structural morphology of the striatum of the mouse of the blank control group (see FIG. 13A) is normal; striatal neurons in the mouse of the solvent group (see FIG. 13B) are degenerated, some cell nuclei (indicated by arrows) are vacuolated, and the arrangement of brain cells is disordered; the overall structure of the striatum of the mouse of the plasminogen administration group (see FIG. 13C) is significantly improved, and is similar to that of the mouse of the blank control group. The results indicate that plasminogen can repair striatal damage in the mouse model of Huntington's disease.

Example 10 Plasminogen Improves Olfactory Nodule Damage in a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]. Preparation of the) 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, and the brain tissue was taken out and fixed in a 10% neutral formaldehyde solution for 24-48 h. The fixed brain tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 3 μm, the slice was subjected to deparaffinage and rehydration, stained with hematoxylin and eosin (HE staining), differentiated with 1% hydrochloride ethanol, returned to blue with ammonia water, dehydrated with graded ethanol, sealed, and placed under a 200×optical microscope, and the olfactory tubercle was observed.

It has been reported that the olfactory tubercle of the mouse model of Huntington's disease is damaged, and patients with Huntington's disease have olfactory deficits^([9]).

The results show that the structural morphology of the olfactory tubercle in the brain of the mouse of the blank control group (see FIG. 14A) is normal; glial cell infiltration (indicated by arrows) in the olfactory tubercle of the mouse of the solvent group (see FIG. 14B) is severe; and glial cell infiltration in the olfactory tubercle of the mouse of the plasminogen administration (see FIG. 14C) group is obviously milder than that of the mouse of the solvent group. The results indicate that plasminogen can improve olfactory tubercle damage in the brain of the mouse model of Huntington's disease.

Example 11 Plasminogen Promotes the Expression of BDNF in the Hippocampus of a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]). Preparation of the 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, and the hippocampus was taken out and fixed in a 10% neutral formaldehyde solution for 24-48 h. The fixed hippocampus tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 3 μm, and the slice was subjected to deparaffinage and rehydration, and washed once with water. The tissue slice was marked by using a PAP pen, incubated in 3% hydrogen peroxide for 15 min, and washed twice with 0.01 M PBS for 5 min each time. The slice was blocked with a 5% normal goat serum (Vector laboratories, Inc., USA) for 30 min; and then, the goat serum was removed, a rabbit anti-BNDF antibody (Boster Biological Technology, PB9075) was added dropwise, and the slice was incubated at 4° C. overnight and washed twice with 0.01 M PBS for 5 min each time. A goat anti-rabbit IgG (HRP) antibody (Vector laboratories, MP-7451) secondary antibody was added, and the slice was incubated at the room temperature for 30 min and washed twice with 0.01 M PBS for 5 min each time. The slice was developed by using a DAB kit (Vector laboratories, Inc., USA), washed three times with water, restained with hematoxylin for 30 s, and rinsed with running water for 5 min. The stained slice was dehydrated with graded ethanol, cleared with xylene, sealed by a neutral gum, and observed under a 400×optical microscope.

Brain-derived neurotrophic factor (BDNF) is a protein synthesized in the brain, is abundant in the central nervous system, and plays an important role in the survival, differentiation, and growth and development of neurons during the development of the central nervous system. BDNF can prevent neuronal damage and death, improve the pathological state of neurons, and promote biological effects, such as regeneration and differentiation, of damaged neurons^([10]).

The results show that a certain amount of BDNF (indicated by arrows) is expressed in the right hippocampus of the mouse of the blank control group (see FIG. 15A); the expression of BDNF in the right hippocampus of the mouse of the solvent group (see FIG. 15B) is slight higher than that of the mouse of the blank control group; the expression of BDNF in the right hippocampus of the mouse of the plasminogen administration group (see FIG. 15C) is obviously higher than that of the mouse of the solvent group, and the statistical difference is close to significant (P=0.07) (see FIG. 15D). The results indicate that damage can stimulate the expression of BDNF, but plasminogen can further promote the expression of BDNF, so as to promote the repair of hippocampal damage in the mouse model of Huntington's disease.

Example 12 Plasminogen Promotes the Expression of BDNF in the Striatum of a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]). Preparation of the 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, the striatum was taken out and fixed in a 10% neutral formaldehyde solution for 24-48 h. The fixed striatum tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The tissue was cut into slices with a thickness of 3 μm, and the slice was subjected to deparaffinage and rehydration, and washed once with water. The tissue slice was marked by using a PAP pen, incubated in 3% hydrogen peroxide for 15 min, and washed twice with 0.01 M PBS for 5 min each time. The slice was blocked with a 5% normal goat serum (Vector laboratories, Inc., USA) for 30 min; and then, the goat serum was removed, a rabbit anti-BNDF antibody (Boster Biological Technology, PB9075) was added dropwise, and the slice was incubated at 4° C. overnight and washed twice with 0.01 M PBS for 5 min each time. A goat anti-rabbit IgG (HRP) antibody (Vector laboratories, MP-7451) secondary antibody was added, and the slice was incubated at the room temperature for 30 min and washed twice with 0.01 M PBS for 5 min each time. The slice was developed by using a DAB kit (Vector laboratories, Inc., USA), washed three times with water, restained with hematoxylin for 30 s, and rinsed with running water for 5 min. The stained slice was dehydrated with graded ethanol, cleared with xylene, sealed by a neutral gum, and observed under a 400×optical microscope.

The results show that a certain amount of BDNF (indicated by arrows) is expressed in the striatum of the mouse of the blank control group (see FIG. 16A); the expression of BDNF in the striatum of the mouse of the solvent group (see FIG. 16B) is slightly higher than that of the mouse of the blank control group; the expression of BDNF in the striatum of the mouse of the plasminogen administration group (see FIG. 16C) is obviously higher than that of the mouse of the solvent group, and the statistical difference is close to significant (P=0.1) (see FIG. 16D). The results indicate that damage can stimulate the expression of BDNF, but plasminogen can further promote the expression of BDNF, so as to promote of the repair of striatal damage in the mouse model of Huntington's disease.

Example 13 Plasminogen Promotes the Regeneration of the Striatal Myelin Sheath in a Mouse Model of Huntington's Disease

3 days before model construction, 6-week-old male C57 mice were weighed and subjected to a simple open field test. The mice were observed for 5 min, spontaneous differences in the random animals were excluded, and finally 23 experimental animals were selected. The mice were randomly divided into two groups, i.e., a blank control group and a model group, according to total travel distances of the mice in the open field test, 6 mice in the blank control group and 17 mice in the model group. 125 μL of PBS was intraperitoneally injected into each mouse of the blank control group, and a 3-nitropropionic acid (3-NP) solution was intraperitoneally injected into each mouse of the model group at a dose of 50 mg/kg (by body weight), twice a day (every 12 h), for 5 consecutive days, to construct models of Huntington's disease^([1]. Preparation of the) 3-NP solution: 3-NP powder (Sigma, catalog number: N5636) was dissolved in PBS to a concentration of 10 mg/mL. On the second day after model construction was completed, which was defined as day 0 of administration, all the mice were weighed and subjected to an open field test. The mice of the model group were randomly divided into two groups, i.e., a solvent control group (9 mice) and a plasminogen administration group (8 mice), according to total travel distances of the mice in the open field test. A solvent (a 10 mM citric acid-sodium citrate solution, pH=7.4) was injected to each mouse of the solvent control group via the tail vein at a dose of 0.1 mL/day, human plasminogen was injected into each mouse of the plasminogen administration group via the tail vein at a dose of 1 mg/0.1 mL/day, and administration was performed for 7 consecutive days. The mice were killed on day 7 of administration, the striatum was taken out and fixed in a 10% neutral formaldehyde solution for 24-48 h. The fixed striatum tissue was dehydrated with graded ethanol, cleared with xylene, and embedded in paraffin. The spinal cord tissue was transversely cut into slices with a thickness of 4 μm, and the slice was subjected to deparaffinage and rehydration, and subjected to LFB staining with a myelin sheath dye. The stained slice was dehydrated with graded ethanol, cleared with xylene, and sealed by a neutral gum. The slice was observed and photographed under an optical microscope.

Luxol fast blue (LFB) staining uses luxol fast blue to stain the myelin sheath, and is an effective method for studying corticospinal tract positioning and myelin sheath lesions, and observing damage to and regeneration and repair of the morphology^([11-12]).

The results show that the structure of the striatal myelin sheath of the mouse of the blank control group (see FIG. 17A) is normal; the striatal myelin protein content in the mouse of the solvent group (see FIG. 17B) is decreased, and cavitation (indicates by arrows) can be observed; the striatal myelin protein content in the mouse of the plasminogen administration group (see FIG. 17C) is obviously greater than that in the mouse of the solvent group, and the statistical difference is close to significant (P=0.09) (see FIG. 17D). The results indicate that plasminogen can promote the formation of striatal myelin protein in the mouse model of Huntington's disease.

REFERENCES

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1. A method for treating Huntington's disease, comprising: administering a therapeutically effective amount of one or more compounds to a subject with Huntington's disease, the one or more compound being selected from: a component of a plasminogen activation pathway, a compound capable of directly activating plasminogen or indirectly activating plasminogen by activating an upstream component of a plasminogen activation pathway, a compound mimicking the activity of plasminogen or plasmin, a compound capable of up-regulating the expression of plasminogen or a plasminogen activator, a plasminogen analog, a plasmin analog, a tPA or uPA analog, and an antagonist of a fibrinolysis inhibitor.
 2. The method according to claim 1, wherein the component of the plasminogen activation pathway is selected from: plasminogen, recombinant human plasmin, Lys-plasminogen, Glu-plasminogen, plasmin, a plasminogen or plasmin variant or analog containing one or more Kringle domains or protease domains of plasminogen or plasmin, mini-plasminogen, mini-plasmin, micro-plasminogen, micro-plasmin, delta-plasminogen, delta-plasmin, a plasminogen activator, tPA, and uPA.
 3. The method according to claim 1, the antagonist of the fibrinolysis inhibitor is an inhibitor of PAI-1, a complement C1 inhibitor, α2 antiplasmin or an α2 macroglobulin, such as an antibody.
 4. The method according to claim 1, wherein the compound has one or more effects on the subject with Huntington's disease, the one or more effects being selected from: improvement or relief of movement disorders, improvement of cognitive impairment, deceleration of weight loss, promotion of the repair of damaged neurons, improvement of neuropsychiatric symptoms, relief of anxiety, reduction of the expression of GFAP in the hippocampus, reduction of apoptosis of hippocampal cells, promotion of recovery of the number of Nissl bodies in cerebellar, hippocampal or striatal neurons, repair of damage to the hippocampus, striatum or olfactory tubercle, promotion of the expression of BDNF in the hippocampus or striatum, and promotion of the regeneration of striatal myelin sheaths.
 5. The method according to claim 1, wherein the compound is used in combination with one or more other drugs or treatment methods.
 6. The method according to claim 5, wherein the other drugs or treatment methods are selected from one or more of: anti-dopaminergic drugs, dopamine receptor inhibitors, antipsychotic drugs (e.g., butyrophenone and phenothiazines), γ-aminobutyrate transaminase inhibitors, cell transplantation therapy, and gene therapy.
 7. The method according to claim 1, wherein the compound is plasminogen.
 8. The method according to claim 1, wherein the plasminogen is human full-length plasminogen or a conservatively substituted variant thereof.
 9. The method according to claim 1, wherein the plasminogen has at least 75%, 80%, 85%, 90%, 95%, 96%, 97%, 98% or 99% sequence identity with sequence 2, and still has the lysine binding activity or the proteolytic activity of plasminogen.
 10. The method according to claim 1, wherein the plasminogen is a protein containing an amino acid sequence having at least 80%, 90%, 95%, 96%, 97%, 98% or 99% amino acid sequence identity with sequence 14 and still having the proteolytic activity of plasminogen.
 11. The method according to claim 1, wherein the plasminogen is selected from Glu-plasminogen, Lys-plasminogen, mini-plasminogen, micro-plasminogen, delta-plasminogen, and variants thereof that retain the proteolytic activity of plasminogen.
 12. The method according to claim 1, wherein the plasminogen contains an amino acid sequence shown as sequence 2, 6, 8, 10 or 12, or contains a conservatively substituted variant of the amino acid sequence shown as sequence 2, 6, 8, 10 or
 12. 13. The method according claim 1, wherein the compound is administered by nasal inhalation, aerosol inhalation, nasal drops, eye drops, ear drops, an intravenous method, an intraperitoneal method, a subcutaneous method, an intracranial method, an intrathecal method, an intra-arterial method (e.g., via the carotid artery) or an intramuscular method. 